Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells

The presence or absence of a phosphorylation on a substrate at any particular point in time is a functional readout of the balance in activity between the regulatory kinase and the counteracting phosphatase. Understanding how stable or short-lived a phosphorylation site is required for fully appreci...

Descripción completa

Detalles Bibliográficos
Autores principales: Rogers, Samuel, McCloy, Rachael A., Parker, Benjamin L., Chaudhuri, Rima, Gayevskiy, Velimir, Hoffman, Nolan J., Watkins, D. Neil, Daly, Roger J., James, David E., Burgess, Andrew
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier 2015
Materias:
Data Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4564385/
https://www.ncbi.nlm.nih.gov/pubmed/26425664
http://dx.doi.org/10.1016/j.dib.2015.08.010
_version_ 1782389417762095104
author Rogers, Samuel
McCloy, Rachael A.
Parker, Benjamin L.
Chaudhuri, Rima
Gayevskiy, Velimir
Hoffman, Nolan J.
Watkins, D. Neil
Daly, Roger J.
James, David E.
Burgess, Andrew
author_facet Rogers, Samuel
McCloy, Rachael A.
Parker, Benjamin L.
Chaudhuri, Rima
Gayevskiy, Velimir
Hoffman, Nolan J.
Watkins, D. Neil
Daly, Roger J.
James, David E.
Burgess, Andrew
author_sort Rogers, Samuel
collection PubMed
description The presence or absence of a phosphorylation on a substrate at any particular point in time is a functional readout of the balance in activity between the regulatory kinase and the counteracting phosphatase. Understanding how stable or short-lived a phosphorylation site is required for fully appreciating the biological consequences of the phosphorylation. Our current understanding of kinases and their substrates is well established; however, the role phosphatases play is less understood. Therefore, we utilized a phosphatase dependent model of mitotic exit to identify potential substrates that are preferentially dephosphorylated. Using this method, we identified >16,000 phosphosites on >3300 unique proteins, and quantified the temporal phosphorylation changes that occur during early mitotic exit (McCloy et al., 2015 [1]). Furthermore, we annotated the majority of these phosphorylation sites with a high confidence upstream kinase using published, motif and prediction based methods. The results from this study have been deposited into the ProteomeXchange repository with identifier PXD001559. Here we provide additional analysis of this dataset; for each of the major mitotic kinases we identified motifs that correlated strongly with phosphorylation status. These motifs could be used to predict the stability of phosphorylated residues in proteins of interest, and help infer potential functional roles for uncharacterized phosphorylations. In addition, we provide validation at the single cell level that serine residues phosphorylated by Cdk are stable during phosphatase dependent mitotic exit. In summary, this unique dataset contains information on the temporal mitotic stability of thousands of phosphorylation sites regulated by dozens of kinases, and information on the potential preference that phosphatases have at both the protein and individual phosphosite level. The compellation of this data provides an invaluable resource for the wider research community.
format Online
Article
Text
id pubmed-4564385
institution National Center for Biotechnology Information
language English
publishDate 2015
publisher Elsevier
record_format MEDLINE/PubMed
spelling pubmed-45643852015-09-30 Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells Rogers, Samuel McCloy, Rachael A. Parker, Benjamin L. Chaudhuri, Rima Gayevskiy, Velimir Hoffman, Nolan J. Watkins, D. Neil Daly, Roger J. James, David E. Burgess, Andrew Data Brief Data Article The presence or absence of a phosphorylation on a substrate at any particular point in time is a functional readout of the balance in activity between the regulatory kinase and the counteracting phosphatase. Understanding how stable or short-lived a phosphorylation site is required for fully appreciating the biological consequences of the phosphorylation. Our current understanding of kinases and their substrates is well established; however, the role phosphatases play is less understood. Therefore, we utilized a phosphatase dependent model of mitotic exit to identify potential substrates that are preferentially dephosphorylated. Using this method, we identified >16,000 phosphosites on >3300 unique proteins, and quantified the temporal phosphorylation changes that occur during early mitotic exit (McCloy et al., 2015 [1]). Furthermore, we annotated the majority of these phosphorylation sites with a high confidence upstream kinase using published, motif and prediction based methods. The results from this study have been deposited into the ProteomeXchange repository with identifier PXD001559. Here we provide additional analysis of this dataset; for each of the major mitotic kinases we identified motifs that correlated strongly with phosphorylation status. These motifs could be used to predict the stability of phosphorylated residues in proteins of interest, and help infer potential functional roles for uncharacterized phosphorylations. In addition, we provide validation at the single cell level that serine residues phosphorylated by Cdk are stable during phosphatase dependent mitotic exit. In summary, this unique dataset contains information on the temporal mitotic stability of thousands of phosphorylation sites regulated by dozens of kinases, and information on the potential preference that phosphatases have at both the protein and individual phosphosite level. The compellation of this data provides an invaluable resource for the wider research community. Elsevier 2015-08-24 /pmc/articles/PMC4564385/ /pubmed/26425664 http://dx.doi.org/10.1016/j.dib.2015.08.010 Text en © 2015 The Authors http://creativecommons.org/licenses/by/4.0/ This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Data Article
Rogers, Samuel
McCloy, Rachael A.
Parker, Benjamin L.
Chaudhuri, Rima
Gayevskiy, Velimir
Hoffman, Nolan J.
Watkins, D. Neil
Daly, Roger J.
James, David E.
Burgess, Andrew
Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title_full Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title_fullStr Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title_full_unstemmed Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title_short Dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
title_sort dataset from the global phosphoproteomic mapping of early mitotic exit in human cells
topic Data Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4564385/
https://www.ncbi.nlm.nih.gov/pubmed/26425664
http://dx.doi.org/10.1016/j.dib.2015.08.010
work_keys_str_mv AT rogerssamuel datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT mccloyrachaela datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT parkerbenjaminl datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT chaudhuririma datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT gayevskiyvelimir datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT hoffmannolanj datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT watkinsdneil datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT dalyrogerj datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT jamesdavide datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells
AT burgessandrew datasetfromtheglobalphosphoproteomicmappingofearlymitoticexitinhumancells

Ejemplares similares